Expression and chromatin structures of cellulolytic enzyme gene regulated by heterochromatin protein 1

Background Heterochromatin protein 1 (HP1, homologue HepA in Penicillium oxalicum) binding is associated with a highly compact chromatin state accompanied by gene silencing or repression. HP1 loss leads to the derepression of gene expression. We investigated HepA roles in regulating cellulolytic enzyme gene expression, as an increasingly number of studies have suggested that cellulolytic enzyme gene expression is not only regulated by transcription factors, but is also affected by the chromatin status. Results Among the genes that exhibited significant differences between the hepA deletion strain (ΔhepA) and the wild type (WT), most (95.0 %) were upregulated in ΔhepA compared with WT. The expression of the key transcription factor for cellulolytic enzyme gene (e.g., repressor CreA and activator ClrB) increased significantly. However, the deletion of hepA led to downregulation of prominent extracellular cellulolytic enzyme genes. Among the top 10 extracellular glycoside hydrolases (Amy15A, Amy13A, Cel7A/CBHI, Cel61A, Chi18A, Cel3A/BGLI, Xyn10A, Cel7B/EGI, Cel5B/EGII, and Cel6A/CBHII), in which secretion amount is from the highest to the tenth in P. oxalicum secretome, eight genes, including two amylase genes (amy15A and amy13A), all five cellulase genes (cel7A/cbh1, cel6A/cbh2, cel7B/eg1, cel5B/eg2, and cel3A/bgl1), and the cellulose-active LPMO gene (cel61A) expression were downregulated. Results of chromatin accessibility real-time PCR (CHART-PCR) showed that the chromatin of all three tested upstream regions opened specifically because of the deletion of hepA in the case of two prominent cellulase genes cel7A/cbh1 and cel7B/eg1. However, the open chromatin status did not occur along with the activation of cellulolytic enzyme gene expression. The overexpression of hepA upregulated the cellulolytic enzyme gene expression without chromatin modification. The overexpression of hepA remarkably activated the cellulolytic enzyme synthesis, not only in WT (~150 % filter paper activity (FPA) increase), but also in the industry strain RE-10 (~20–30 % FPA increase). Conclusions HepA is required for chromatin condensation of prominent cellulase genes. However, the opening of chromatin mediated by the deletion of hepA was not positively correlated with cellulolytic enzyme gene activation. HepA is actually a positive regulator for cellulolytic enzyme gene expression and could be a promising target for genetic modification to improve cellulolytic enzyme synthesis. Electronic supplementary material The online version of this article (doi:10.1186/s13068-016-0624-9) contains supplementary material, which is available to authorized users.


Background
Lignocellulolytic enzymes are industrially important enzymes, particularly in the textile or paper industry. In the production of cellulosic ethanol, lignocellulolytic enzymes are applied to break down lignocellulosic material to release d-glucose, which can subsequently be used in the sugar-to-ethanol fermentation by yeast. The costs of the necessary enzymes during this process have a huge influence on the price and competitiveness of the end-product [1]. Some filamentous fungi, such as Trichoderma reesei [2], Aspergillus niger [3], Neurospora crassa [4], and Penicillium oxalicum [5], can secrete a complex

Open Access
Biotechnology for Biofuels *Correspondence: qinyuqi@sdu.edu.cn 1 National Glycoengineering Research Center and State Key Lab of Microbial Technology, Shandong University, Jinan 250100, China Full list of author information is available at the end of the article arsenal of enzymes that synergistically deconstructs lignocellulosic material. Research on the regulation of cellulolytic enzyme gene expression may be very useful in increasing the production of these enzymes in their native hosts.
Cellulolytic enzyme production is tightly controlled at the transcriptional level in fungi. Several transcriptional activators (i.e., orthologous XlnR/Xyr1 and ClrB/ Clr2) [6,7] and repressors (i.e., orthologous CreA/Cre1) [8] participate in the process. Transcription factors are currently thought to induce the reorganization of local chromatin in eukaryotes; activators recruit nucleosome modifiers that help transcriptional machinery bind at the promoter or initiate transcription [9]. Two types of nucleosome modifiers exist, those that remodel the nucleosomes, such as ATP-dependent activity of SWI/ SNF [10], and those that add chemical groups to the tails of histone, such as histone methyltransferases or histone acetyltransferases [11]. This modification can "loosen" the chromatin structure, rendering it accessible and capable of binding the transcriptional machinery [12]. For example, the helicase gene snf2, which is a component of yeast Swi/Snf multisubunit chromatin remodeling complex, was found to be upregulated significantly in T. reesei Δcre1 mutant and thought to be involved in the cellulase gene repression by Cre1 at a high growth rate [13]. Another chromatin-associated protein (T. reesei ID 107641), which has a bromodomain, a module found in many chromatin-associated proteins and which plays a key role in chromatin remodeling, was reported to bear the highest expression in T. reesei Δcre1 when the strain was cultivated in cellulose and is thought to result in an alteration of chromatin structure that consequently change the expression of genes related to lignocelluloses degradation [14]. Histone acetyltransferase Gcn5 has also been proven to be required in the induction expression of cellulase genes in T. reesei, with acetylation of K9 and K14 of histone H3 in the cellulase gene promoter dramatically affected in the absence of Gcn5 [15]. The lysines of histones H3 are usually acetylated in transcriptionally active chromatin, and usually hypoacetylated in transcriptionally repressed or silent chromatin [16]. The lack of acetylation enables the mono-, di-, or tri-methylation of H3K9 (H3K9me) by histone methyltransferase, such as Clr4 [17]. This histone modification could be recognized by the heterochromatin protein 1 (HP1) [18].
HP1, a small non-histone chromosomal protein, was first identified in Drosophila melanogaster as a dominant suppressor of position-effect variegation (PEV) on heterochromatin gene silencing [19]. HP1 protein binding is always associated with highly compact chromatin state accompanied by gene silencing or repression, whereas its loss leads to the derepression of gene expression. The best-studied fungal HP1 homologues in fungi were the Schizosaccharomyces pombe SWI6 (reviewed in [20]), N. crassa Hpo [21], and Aspergillus nidulans HepA [22]. N. crassa Hpo specifically binds H3K9me3, recruits DNA methyltransferase DIM-2, and forms distinct DNA methylation complexes involved in gene repression or gene silencing [21]. S. pombe SWI6 interacts with and recruits H3K9 methyltransferase Clr4, and plays a role in the establishment and maintenance of heterochromatin [18]. The heterochromatinization mediated by HepA/Clr4 was counteracted by LaeA (ortholog of Lae1) in A. nidulans [22]. LaeA is a putative methyltransferase considered to be a positive regulator for glycoside hydrolase gene expression because its overexpression improves cellulase gene transcription, whereas a complete loss of expression of all seven cellulases and auxiliary factors for cellulose degradation was observed in the T. reesei lae1 deletion strain [23]. The deletion of hepA upregulated laeA expression; whereas LaeA prevented HepA binding and the formation of repressive chromatin [22], suggesting that HepA might be involved in cellulolytic enzyme gene expression. Thiago also found that HP1 gene expression was downregulated significantly when T. reesei QM6a was cultivated in a sophorose medium, which is an induction medium for cellulolytic enzyme gene expression, compared with that in glucose repression medium [24]. Therefore, a possible speculation could be that HepA might be a negative regulator for cellulolytic enzyme gene expression.
To determine whether HepA participates in gene expression, especially in cellulolytic enzyme gene expression in filamentous fungi, the hepA gene was deleted and overexpressed in P. oxalicum, which is a strain used in industrial-scale glycoside hydrolase production [25,26]. As no report has been made on the positive roles of HP1 in filamentous fungi, it is rather surprising that the deletion of hepA indicated the repression of cellulolytic enzyme gene, whereas the overexpression of hepA exhibited obvious activation of cellulolytic enzyme synthesis not only in a wild-type (WT) strain, but also in an industry strain. The unexpected results showed that HepA is actually a positive regulator for cellulolytic enzyme gene expression. We found that HepA is required for chromatin condensation using chromatin accessibility real-time PCR (CHART-PCR). However, the opening of chromatin in the absence of HepA did not occur with the activation of gene expression, suggesting that chromatin condensation or decondensation in the core promoter region alone does not repress or activate gene expression.

Identification of P. oxalicum HepA
Similar to S. pombe and N. crassa, P. oxalicum contains only one HP1 homologue, HepA. P. oxalicum HepA contains 241 amino acids of two conserved domains according to the Pfam analysis [27]. One is a 54-amino-acid N-terminal chromatin organization modifier domain (CHD), and the other is a 58-amino-acid C-terminal chromo shadow domain (CSD). These domains are joined by a flexible hinge (Fig. 1a). The CHD is involved in the interaction with H3K9-methylated nucleosomes required for chromatin binding, whereas CSD mainly mediates interaction with other heterochromatin proteins [28]. HP1 is phylogenetically conserved and found in almost all eukaryotes, with the exception of budding yeast. P. oxalicum HepA exhibits a limited overall identity (28 %) to S. pombe SWI6, an identity (35 %) to N. crassa Hpo, and a higher identity (43 % identity) to A. nidulans HepA. The phylogenetic trees indicate the evolution of HepA (Fig. 1b).

Diminished cellulolytic halo was observed around the ΔhepA colony
The ΔhepA colony appeared greenish-brown compared with the dark-green WT and complemented strains when the strains were grown on potato dextrose agar (PDA) (Fig. 2a). The levels of conidiation in the ΔhepA mutant were significantly reduced (~23.3 % of WT) after five days of cultivation on PDA (Fig. 2b). Either expressions of P. oxalicum hepA (RPohepA) or A. nidulans hepA (RAnhepA) could recomplement the defect in ΔhepA (Fig. 2), indicating that the biological roles of A. nidulans HepA and P. oxalicum HaeA were well-conserved. The radial growth and conidiation of ΔhepA were identical to that of the WT when the strains were grown on VMM + glucose agar, which is in contrast with the S. pombe and N. crassa studied so far, in which HP1 deletion was shown to affect viability strongly. The mutations in N. crassa Hpo showed pronounced defects in asexual spore and aerial hyphae formation [29]. No cellulolytic halo was observed around the ΔhepA colony when the strains were grown on VMM + cellulose agar, whereas a clear cellulolytic halo was found around the WT colony, suggesting that the deletion of hepA suppressed cellulolytic enzyme formation.

Transcriptome data showed that deletion of hepA led to downregulation of prominent extracellular cellulolytic enzyme genes
The unexpected observation of diminished cellulolytic halo around the ΔhepA colony led us to exploit the role of HepA in regulating cellulolytic enzyme gene expression. WT and ΔhepA were cultivated in cellulose and wheat bran medium, which is an optimum medium for cellulolytic enzyme formation, to obtain a global view of the effect of hepA deletion on gene expression, especially the cellulolytic enzyme gene expression. The mRNAs from WT and ΔhepA at cultivation time of 48 h were subjected to high-throughput Illumina sequencing (Realbio, Shanghai, China) to obtain the transcriptome of WT and ΔhepA. More than 10 million reads were obtained for each sample. The copy number of unambiguous reads (tags mapped to one single gene) for each gene was normalized to reads per kilobases per million reads (RPKM) clean reads. Saturation analysis indicated that the capacity of the two libraries approached saturation (Additional file 1: Fig. S1). A genome-wide transcriptome analysis revealed the extensive expression of the entire P. oxalicum genome. Among the 10,021 protein-coding genes predicted in the genome database, 9016 (90.0 %) and 9361 (93.4 %) genes were expressed in WT and ΔhepA, respectively. The genes of significantly differential expression levels were identified through a significance test with combined thresholds (FDR ≤ 0.001 and fold change ≥2) [30]. Blast2GO was used for the function enrichment analysis of gene sets with a threshold of FDR ≤ 0.05 [31].
Transcriptome data showed that the expression levels of 1654 genes exhibited significant differences (twofold or greater, FDR < 0.001) between the ΔhepA and WT. In the regulon, 1571 genes (95.0 %) were upregulated in ΔhepA compared with the WT. As expected, the vast majority of genes expression was upregulated in ΔhepA because HepA othologs (HP1 and Swi6) are always associated with gene repression or silencing. HP1 targeting results in a quantifiable degree of chromatin condensation and repressed genes, whereas the loss of HP1 disrupts repression completely [32]. GO enrichment analysis revealed that the upregulated genes in ΔhepA were involved mainly in amino acid binding, amino acid transmembrane transporter activity, ATP-dependent helicase activity, oxidoreductase activity acting on CH-OH group of donors, RNA methyltransferase activity, rRNA binding, and structural constituent of ribosome compared with that in WT (Fig. 3a, red bars). The GO terms which included most abundant genes in cellular component, biological process, and molecular function are translation, oxidation-reduction process, and oxidoreductase activity, respectively. For example, 118 ribosomal protein genes and 44 rRNA processing genes were enriched ( Fig. 3; Additional file 2: Table S1), suggesting possible upregulation of protein synthesis in ΔhepA. The upregulated genes (GO category: molecular function) and their predicted functions are listed in the Additional file 2: Table S1.

Overexpression of hepA activated cellulolytic enzyme synthesis remarkably
We doubted the ability of the hepA overexpression to activate the cellulase synthesis because the prominent extracellular cellulolytic enzyme gene expression was downregulated in ΔhepA, and HP1 has consistently been reported with dose-dependent effect on gene expression [34]. Two overexpression strains (OEhepA-1 and OEhepA-2, hepA overexpressed under gpdA strong constitutive promoter), which were selected randomly, indicated clearer hydrolysis halos than that of WT (Fig. 4a) when the strains were grown on VMM + starch or VMM + cellulose agar, suggesting higher amylase or cellulolytic enzyme activity in OEhepA. Pure cellulose was used as the sole carbon source for the agar. We cultivated the WT, ΔhepA, and OEhepA in a submerged medium with wheat bran and cellulose because complex carbon sources from plant materials are more efficient than pure cellulose in promoting the expression of cellulolytic enzyme. The supernatants from the WT and mutants were profiled by SDS-PAGE (Fig. 4b). Equal volumes of supernatants were loaded. Significantly fainter protein bands were detected in ΔhepA than in WT, whereas darker protein bands were detected in OEhepA, especially in the range of 40-116 kDa, which is an area for the aggregation of glycoside hydrolases in particular. Most prominent glucoamylases, cellobiohydrolases, endoglucanases, and β-glucosidases were located in the area according to previous reports [33].
Were the changes in cellulolytic enzyme synthesis in the mutants caused by their different biomass levels? Performing an assay of the mycelia biomass according to the dry cell weight can be difficult, because wheat bran and cellulose were added in the fermentation medium as inducer and unconsumed wheat bran and cellulose interfered with the results. Thus, total intracellular protein concentration was determined to indicate the biomass. Except for some differences at the early state of cultivation (4 h), identical intracellular protein concentrations were observed in WT, ΔhepA, OEhepA, RPohepA, and RAnhepA after 24 h of cultivation, indicating that the reduced cellulolytic activities in ΔhepA or increased cellulolytic enzyme activities in OEhepA were not correlated with the biomass level (Additional file 5: Fig. S4).

Cellulolytic enzyme gene expression and chromatin structures are regulated by the HepA
A quantitative PCR was carried out to compare the transcription patterns of the cellulase genes, including the prominent cellobiohydrolase gene cel7A/cbh1 and endoglucanase gene cel7B/eg1 (Fig. 6). The transcript levels of cel7A/cbh1 and cel7B/eg1 in both hepA overexpression strains obviously and significantly increased. For OEhepA-1, the transcript level of cel7A/cbh1 increased by 3.8-and 6.5-folds at 24 and 48 h compared with  (Fig. 6a). The transcript level of cel7B/eg1 increased by 51.3-and 11.0-folds at 24 and 48 h compared with the WT, respectively (Fig. 6b). The results suggested that overexpression of hepA significantly activated the cellulolytic enzyme gene expression.
Transcriptional activation in eukaryotes is often accompanied by alterations in the chromatin structure at specific regulatory sites. We used CHART-PCR analysis to better comprehend the contribution of HepA to the changes in chromatin packing, especially the chromatin status of the core promoter and upstream region of cellulolytic enzyme gene. We first analyzed the upstream sequence and core promoters for cel7A/cbh1 and cel7B/eg1. Eukaryotic core promoter refers to the minimal set of sequence elements required for accurate transcription initiation by the Pol II machinery. The initiator element (Inr) is the most common element found in combination with both TATA element (or box) and downstream promoter element (DPE) [35]. The Inr (CCATTCC) and TATA box (TATATAA) were found in the cel7A Pol II core promoter region (Fig. 7a), fitting with the consensus sequence of Inr (C/T) 2   and TATA element (TATAAGT) were found in the cel7B Pol II core promoter region (Fig. 7b), with base variation (indicated by the asterisk) compared with the consensus sequence of Inr and TATA box. Both cel7A and cel7B bore the putative CreA-binding sites "5′-GGC(T/A) 3 -3′" [8] and putative XlnR-binding sites "5′-SYGGRG-3′" [36]. DPE elements were not found in both cel7A and cel7B. Three regions were designed for the CHART-PCR of cel7A/cbh1 and cel7B/eg1. In the cel7A/cbh1 upstream region, region 1 (+5 to −142), region 2 (−143 to −303), and region 3 (−330 to −470), were designed, respectively. In the cel7B/eg1 upstream region, region 1 (+35 to −138), region 2 (−164 to −341), and region 3 (−369 to −539), were designed, respectively. Region 1 covered the core promoters region; Regions 2 and 3 were upstream the core promoters, which were considered for transcriptional regulatory protein (i.e., activator XlnR or repressor CreA) binding (Fig. 7a, b).
Next, we analyzed the chromatin status change mediated by HepA. In the ΔhepA mutant, the chromatin of all three tested upstream regions opened specifically in the cases of cel7A/cbh1 and cel7B/eg1. The chromatin accessibility index increased remarkably (Fig. 7c, d). The results suggested that HepA was required for chromatin condensation, but this action was not essential for the repression of transcription because the opening of chromatin in the absence of HepA did not occur with the increase of gene expression (Fig. 6). Meanwhile, transcripts can even be detected at high levels in the hepA overexpression strain although the chromatin status of OEhepA was identical with that of WT. Chromatin closing or opening alone does not repress or activate gene expression. Among the three target regions for either cel7A/cbh1 or cel7B/eg1 in the ΔhepA mutant, region 1 showed the most relaxed chromatin status. The farther the regions were from the core promoters, the lower the opening degree of chromatin. Considering that region 1 covered the core promoter region, the result was expected because the disruption of the chromatin structure from the core promoter region or the proximal promoter region of a gene is a prerequisite to transcription initiation and elongation [37].

Overexpression of hepA improved cellulase activity in the industrial strain RE-10
P. oxalicum has been used in the industrial production of cellulase. We overexpressed the hepA gene in the industrial strain RE-10 to enhance the cellulolytic enzyme synthesis of the P. oxalicum further. RE-10, with an improved 20-fold filter paper activity compared to P. oxalicum WT 114-2, included three genetic modifications: deletion of transcription repressor CreA, overexpression of transcription activator ClrB, and deletion intracellular β-glucosidase Bgl2 [26]. The overexpression of hepA can improve cellulase activity in the industrial strain RE-10. Both overexpression strains (RE-10::OEhepA-1 and RE-10::OEhepA-2), which were selected randomly, showed improved cellulase activity than RE-10. After 5 days of cultivation, the filter paper activities of RE-10::OEhepA-1 and RE-10::OEhepA-2 were 5.34 and 5.83 IU/mL, which increased by 20.8 and 31.9 % compared with that of RE-10, respectively (Fig. 8).

Discussion
According to our initial speculation, HepA might be a negative regulator for cellulolytic enzyme gene expression, as HP1 binding have always been implicated in heterochromatin formation and gene repression, whereas its loss leads to derepression of gene expression [20]. Therefore, we observed rather surprisingly that HepA is actually a positive regulator for the cellulolytic enzyme gene expression because the deletion of hepA showed the repression of cellulolytic enzyme gene expression, whereas the overexpression of hepA indicated an obvious activation of cellulolytic enzyme gene expression. Indeed, in addition to the prominent roles of HP1 in gene repression, increasing evidence supports the view that HP1 proteins play a positive role in transcription. HP1 is not only required for the proper expression of genes that reside within the heterochromatin, but is also required for the expression of several euchromatic genes [40]. For example, many genes, such as cdc2, located in euchromatin are downregulated in the HP1 mutant Drosophila [41]. Reduced HP1 dosage leads to lower level of heat shock gene mRNA, whereas HP1 overexpression leads to increased hsp70 mRNA [42]. However, no report has been made on the positive roles of HP1 in filamentous fungi. The involvement of N. crassa Hpo in heterochromatin formation, DNA methylation, and gene silencing has been reported [43]. The deletion of hepA in A. nidulans upregulated the SM gene expression; HepA occupancy at the ST cluster decreased during the transcriptional activation [22] and was required for transgene silencing [44]. Our results also showed that the vast majority (95.0 %) of genes that exhibited significant differences between ΔhepA and WT were upregulated in ΔhepA compared with those in WT (Fig. 3), suggesting that HepA played a main negative role in transcription.
The positive regulation of the cellulolytic enzyme gene expression by HepA was an unexpected finding.
Although numerous studies have been conducted to elucidate the mechanism of the transcriptional regulation of cellulolytic enzyme genes by transcription regulatory proteins, few studies have been conducted to investigate the effect of chromatin status on their expressions. In the generally accepted model, transcriptionally repressed chromatin is condensed and transcriptionally active chromatin is decondensed. For example, in T. reesei strain bearing a xyr1 deletion, the sophorose-mediated inductions of the two prominent cellulase-encoding genes cbh1 and cbh2 expressions are lost and the degrees of chromatin opening are strongly reduced [24]. CreI was also reported to play an essential role in correct nucleosome positioning within the main cellulase gene cbh1 promoter [45].
The interaction between HP1 and chromatin was speculated to be static; HP1 acted as "molecular glue" locking nucleosomes together tightly, triggering a repressive chromatin structure once it is targeted to specific promoters, thereby blocking the access of the transcription machinery or activators to the gene [46]. However, our results on the prominent cellulase gene cbh1 and Fig. 9 Expression levels of the creA, clrB, and bgl2 in WT and different mutants determined using qPCR. a creA, b clrB, and c bgl2. There is no data for creA and bgl2 expression in RE-10, RE-10::OEhepA-1, or RE-10::OEhepA-2, as both creA and bgl2 were deleted in RE-10 eg1 expressions and the results of CHART-PCR did not fit the classical view of chromatin structures and gene expression. In particular, we found that the deletion of hepA led to highly opened chromatin, without increase for cellulolytic enzyme gene expression. The overexpression of hepA led to the active cellulolytic enzyme gene but without chromatin structure modification. These results suggest that chromatin condensation or decondensation in the promoter region alone does not repress or activate gene expression. The opening of chromatin was not always positively correlated with gene expression, but showed considerable variety in different genes and cultures. In T. reesei QM6a-CreI 96 (a truncated CreI having left a sequence that would only encode for one of the two zinc finger regions of CreI, 96 aa long), the cbh1 and cbh2 gene expressions increased with simultaneous opening of chromatin during the strain on d-Glucose. No direct correlation between gene expression and chromatin accessibility was observed in the QM6a-ΔCreI strain, and no correlation of gene expression was observed in either QM6a-CreI 96 or QM6a-ΔCreI with the simultaneous opening of chromatin in the strains during sophorose induction [47]. Some studies have shown that the repression or silencing of genes is not caused by the physical inaccessibility of condensed chromatin domains to transcription factors; compact chromatin domains are readily accessible to large macromolecules, such as protein and dextrans [48]. The silent chromatin in S. pombe also exhibits high MNaseI sensitivity [49]; chromatin condensation is independent of HP1 homologue Swi6, although most gene silencing disappear at the subtelomeric region in the Δswi6 mutant [50]. Interestingly, GO analysis showed downregulation of extracellular cellulolytic enzyme genes, along with upregulation of genes involved in protein synthesis and downregulation of one secondary metabolic gene cluster. The research by Arvas showed that T. reesei genes involved in major biosynthetic activities such as protein synthesis and energy-related genes, were negatively correlated with extracellular specific protein production rate (SPPR), while genes of secondary metabolism were positively correlated with SPPR [51]. So, the decreased cellulase activity in ΔhepA might be along with possible derepression of translation machinery the same as described by Arvas et al.
Although the overexpression of hepA in WT could lead to two to threefold improvement of PFA, the overexpression of hepA in the industry strain RE-10 only brought 20-30 % improvement of PFA. RE-10 is a genetic modification strain bearing the deletion of transcription repressor CreA, overexpression of transcription activator ClrB, and deletion of intracellular β-glucosidase Bgl2 [26]. Although CreA/Cre1 and ClrB/Clr2 are prominent for their functions in cellulolytic enzyme gene expression regulation [6,7], their regulons are not limited to cellulolytic enzyme genes. T. reesei Cre1 plays a major role in the regulation of 250 genes, including cellulolytic enzyme genes and genes linked to transcription regulation (e.g., the helicase SNF2 involved in chromatin remodeling and the transcriptional regulator MedA involved in sporulation) [13]. P. oxalicum CreA and ClrB were reported to be involved in the regulation of at least 1100 and 220 genes, respectively. Furthermore, the simultaneous overexpression of ClrB and lack of CreA caused stronger synergistic effect on gene expression, affecting more than 2000 genes [38], including 429 genes, which were also detected in the regulon of hepA deletion strain (data not shown). These genes not only included cellulolytic enzyme gene, but also some transcription factors encoding genes, such as the brlA (PDE_00087) involved in both sporulation and cellulase formation [52], and Rho GTPase encoding gene rhoC1 (PDE_03690) involved in G-protein-mediated signal transduction and associated with hemicellulose degradation [53,54]. Some genes, which are attributed to the improvement of cellulolytic enzyme gene expression regulated in OEhepA, overlapped with the genes regulated in RE-10. This overlapping might be the reason the overexpression of hepA in RE-10 did not lead to so significant improvement like that of the overexpression of hepA in WT.
HepA is obviously involved in cellulolytic enzyme gene expression, and HepA could be a promising target for genetic modification to improve cellulolytic enzyme synthesis. However, the mechanisms of HepA-mediated cellulolytic enzyme gene activation are not fully understood. No difference of the creA, clrB, or bgl2 expression was observed between WT and OEhepA, suggesting that the activation of the cellulolytic enzyme gene expression in the hepA overexpression strain was not attributed to the above three regulators. In A. nidulans, HepA and histone methyltransferase Clr4 form protein complex involving in gene repression [22]. Interestingly, in the screen for P. oxalicum LaeA (a putative histone methyltransferase) interaction protein in yeast two-hybrid library, HepA was one of the screened proteins that interacted with LaeA (self-communication, data unpublished). LaeA, as a positive regulator of cellulolytic enzyme gene [23], can prevent HepA binding and the formation of repressive chromatin [22]. LaeA's partner VeA is also involved in cellulase gene expression [55]. Whether HepA can interact with LaeA (just like Clr4) and form the complex in vivo? Therefore, additional genetic analysis of the integration of HepA and LaeA, and additional biochemical analysis of HepA-containing complexes could provide insights into its role in cellulolytic enzyme gene activation.

Conclusions
The results obtained in this study indicate that HepA is required for chromatin condensation of prominent cellulase genes. However, the opening of chromatin mediated by the deletion of hepA was not positively correlated with cellulase gene activation. The activation of cellulase gene caused by hepA overexpression did not go along with the chromatin status modification. The results suggested that chromatin condensation or decondensation alone in the promoter region does not repress or activate gene expression. HepA is a positive regulator for cellulolytic enzyme gene expression and could be a promising target for genetic modification to improve cellulolytic enzyme synthesis.

Genetic manipulations
We constructed deletion and overexpression cassettes with double-joint PCR [56]. WT genomic DNA was used as the template of the 5′-and 3′-flanking regions of hepA gene (1767 and 1499 bp, respectively) with primer pairs DhepA-UF/DhepA-hph-UR and DhepA-hph-DF/ DhepA-DR to construct the hepA deletion strain. The marker gene hygromycin B (hph) (2425 bp) was amplified from plasmid Psilent1 [57] using primer pairs hph-F/ hph-R. The three PCR fragments were fused with fusion PCR. The products were then amplified using nest primer pairs DhepA-NF/DhepA-NR. The PCR products (4826 bp) were transformed into WT to obtain ΔhepA. We used primer pairs RhepA-F/RhepA-R to obtain intact hepA sequence (open reading frame, 5′-flanking regions including promoter region, and 3′-flanking regions including terminator sequence) 2219 bp and complement the ΔhepA mutant with the P. oxalicum WT hepA. The resistant gene pyrithiamine (ptrA) was amplified from plasmid pME2892 [58] using primer ptra-F/ptra-R. The two fragments were fused and amplified using nest primer RhepA-NF/RhepA-NR. The PCR products (4068 bp) were transformed into ΔhepA to obtain the complement strain RPohepA. We used the primer pairs ANhepA-F/ANhepA-R to obtain intact hepA sequence (open reading frame, 5′-flanking regions including promoter region, and 3′-flanking regions including terminator sequence) 2339 bp to complement the ΔhepA mutant with the A. nidulans hepA. The marker gene ptrA was also amplified from plasmid pME2892. The two PCR fragments were fused and amplified using nest primer ANhepA-NF/ANhepA-NR. The PCR products (4274 bp) were transformed into ΔhepA to obtain complement strain RAnhepA. To construct the hepA overexpression strain in WT, the primers OEhepA-F/OEhepA-R, gpdA-F/gpdA-R, and hph-F/hph-R were used to obtain hepA open reading frame and 3′-flanking regions, including terminator sequence (1346 bp), the gpdA (glyceraldehyde-3-phosphate dehydrogenase) promoter (1256 bp), and resistant gene hygromycin B (hph) (2425 bp), respectively. The three PCR fragments were fused and amplified using nest PCR primer OEhepA-NF/OEhepA-NR. The PCR products (4595 bp) were transformed directly into P. oxallicum 114-2 to obtain OEhepA. The promoter region of the gene PDE_02864, which encodes 40S ribosomal protein S8 [38], was amplified with primer pairs DF/DR (1872 bp) to construct the hepA overexpression strain in the industry strain P. oxalicum RE- 10. The open reading frame of hepA was amplified with primer REhepA-F/REhepA-R. The fragments were fused and amplified using nest primer RE-NF/RE-DR. The PCR products (6482 bp) were transformed into RE-10 to obtain RE-10::OEhepA. All primers used are provided in the Additional file 6: Table S2.
The transformations constructed in this study were further confirmed by Southern blot using a DIG Easy Hyb kit (Roche Diagnostics, Germany) based on the manufacturer's protocol. Genomics DNA was digested with the restriction of endonuclease and separated from 0.75 % agarose gel electrophoresis. The DNA was transferred to the Hybond-N + nylon membranes (Amersham Biosciences/GE Healthcare, USA). Primer DhepA-SF/ DhepA-SR, OEhepA-SF/OEhepA-SR, RpohepA-SF/Rpo-hepA-SR, and RanhepA-SF/RanhepA-SR were used to amplify the probe from the P. oxallicum 114-2 genomics DNA to verify the hepA deletion (ΔhepA), hepA overexpression (OEhepA), P. oxalicum hepA complement (RPo-hepA), and A. nidulans hepA complement (RAnhepA) strains, respectively. The hybridization DNA sizes in WT and genetic manipulate strains were different. All primers used are provided in the Additional file 6: Table S2. The strategy and results of Southern blot are provided in the Additional file 7: Figure S5.

Cellulolytic activity assay
For fermentation, VMM added glucose (2 %, w/v) was used for hyphal growth for 22 h at 30 °C. The mycelia were then harvested by vacuum filtration, and 0.3 g of mycelia was transferred into a 50 mL fermentation medium.

Transcriptome assay and GO analysis
The culture method was similar to that described in the part of "cellulolytic activity assay. " After 48 h of cultivation, total RNA was extracted from the frozen mycelia after lyophilization using the RNAisoTM reagent (TaKaRa, Dalian, China) and incubated with 10 U DNase I (Takara, Dalian, China) for 30 min at 37 °C to remove genomic DNA. Transcriptome assay based on Illumina sequencing was performed by Realbio (Realbio, Shanghai, China). Sequenced reads were mapped against predicted transcripts from the P. oxalicum 114-2 genome using SOAP2 software for short oligonucleotide alignment (http://www.soap.genomics.org.cn/soapaligner.html). Transcript abundance (reads per Kb per million reads, RPKM) [59] genes with significantly different expression levels were identified through a significance test with combined thresholds (FDR ≤ 0.001 and fold change ≥2) [30]. Blast2GO was used for function enrichment analysis of the gene sets with threshold at FDR ≤ 0.05 [31].

qRT-PCR analysis
The culture method was similar to that described in the part of "cellulolytic activity assay. " After 4, 24, and 48 h of cultivation, the total RNA was extracted using the Trizol reagent (TaKaRa, Japan) and cDNA synthesis was performed using the PrimeScript RT reagent Kit (TaKaRa, Japan). Primers CBH-QF/CBH-QR, EG-QF/EG-QR, creA-QF/creA-QR, clrB-QF/clrB-QR, and bgl2-QF/bgl2-QR were used to amplify cel7A/cbh1, cel7B/eg1, creA, clrB, and bgl2, respectively. Quantitative PCR was performed on Roche 480 Light-Cycler (Roche, Mannheim, Germany) using SYBR Premix Ex Taq ™ (TaKaRa, Japan). Three biological replicates and two experiment replicates were required for one sample. Actin gene was used for data normalization. Primers used in the qRT-PCR analysis are listed in the Additional file 6: Table S2.

Chromatin accessibility real-time PCR (CHART-PCR)
CHART-PCR assay was performed according to the methods described by Mello-de-Sousa [47]. Spores of WT, ΔhepA mutant, and OEhepA strains were cultivated on wheat bran extract agar slants at 30 °C for 5 days, and washed by 0.9 % NaCl with 0.1 % Tween 20. The spore suspension was transferred into a 1× Vogel's medium with 2 % glucose as the carbon source for 22 h. The mycelia were harvested by vacuum filtration, and portions (0.3 g) were transferred into a 50 mL medium containing 1× Vogel's medium with 1 % wheat bran and 1 % microcrystalline cellulose as carbon source. The samples from 24 h after induction were collected and ground in liquid nitrogen. Then, 100 mg of powder was pushed into 1 mL of nuclease digestion buffer (250 mM sucrose, 60 mM KCl, 15 mM NaCl, 0.05 mM CaCl 2 , 3 mM MgCl 2 , 0.5 mM DTT, and 15 mM pH 7.5 Tris-HCl). Subsequently, 10 μL RNase-free DNase I (TaKaRa Biotechnology) was added to 100 μL samples at 37 °C for 5 min. The reaction was stopped by adding 100 μL of termination buffer with 20 mM EDTA and 2 % SDS. The same amounts of phenol-chloroform and chloroform were added for protein extraction. The supernatant was treated with 2 μL 1 mg/ mL RNaseA at 37 °C for 15 min. The DNA was precipitated with 0.3 M NaAc and two volumes of ethanol. The DNA was then suspended with 20 μL of double-distilled water. qPCR analysis of the DNase I-treatment samples was performed to measure the relative abundance of target regions. Primers CBH1-F2/CBH1-R2, CBH1-F3/CBH1-R3, and CBH1-F4/CBH1-R4 were used to amplify the cel7A/cbh1 upstream region 1 (+5 to −142), region 2 (−143 to −303), and region 3 (−330 to −470), respectively. Primers EG1-F1/EG1-R1, EG1-F2/EG1-R2, and EG1-F3/EG1-R3 were used to amplify the cel7B/eg1 upstream region 1 (+35 to −138), region 2 (−164 to −341), and region 3 (−369 to −539), respectively. qRT-PCR was performed using SYBR Premix Ex Taq (Perfect Real-time, TaKaRa Biotechnology) with a LightCycler 480 system and software Version 4.0 (Roche, Mannheim, Germany). Each sample was prepared in triplicate. The chromatin accessibility index (CAI) was defined as CAI = 1/ Ds/Dc, where Ds is the amount of intact DNA detected for each target region and Dc is the amount of intact DNA detected for the promoter regions of housekeeping gene sar1. The amount of intact DNA was calculated by comparing the threshold values of PCR amplification plots with the standard curve generated for each primer set using serial dilutions of genomic, uncut DNA. All primers used are listed in the Additional file 6: Table S2.